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蓖麻毒素-胶体金偶联物在非洲绿猴肾细胞中的受体介导内吞作用。内吞后在细胞内运输至内体系统的液泡和管状小泡部分。

Receptor-mediated endocytosis of a ricin-colloidal gold conjugate in vero cells. Intracellular routing to vacuolar and tubulo-vesicular portions of the endosomal system.

作者信息

van Deurs B, Pedersen L R, Sundan A, Olsnes S, Sandvig K

出版信息

Exp Cell Res. 1985 Aug;159(2):287-304. doi: 10.1016/s0014-4827(85)80003-3.

Abstract

We have prepared a conjugate (Ri-Au) of the toxic plant protein ricin and colloidal gold (particle size 5 nm) and used it for internalization studies in monolayer cultures of Vero cells. The Ri-Au conjugate was very stable, with only little release of ricin ([125I]Ri) from the gold particles within a pH range of 4.5-8.0. Within 2 h at 37 degrees C, only very little intracellular degradation of the ricin preparation ([125I]Ri-Au) occurred. The cells bound the same proportion of native ricin ([125I]Ri) and Ri-Au from the medium, and the kinetics of toxicity (decrease in cellular incorporation of [3H]leucine) of [125I]Ri and [125I]Ri-Au were also comparable. At 4 degrees C, the cell-surface binding of Ri-Au was continuous and distinct, as revealed by electron microscopy. This binding was specific, since almost no Ri-Au surface binding occurred at 4 degrees C in the presence of 0.1 M lactose or 1 mg/ml native (unlabelled) ricin. Within the first 30 min of warming prelabelled cells to 37 degrees C, the amount of surface-associated Ri-Au decreased considerably (from 150 to 60 gold particles per micron cell surface in 40 nm sections). Coated pits and vesicles were involved in the internalization of Ri-Au, and within 5-30 min at 37 degrees C Ri-Au had been delivered to vacuolar and tubulo-vesicular portions of the endosomal system, and later also to lysosomes. Analysis of very thin (ca 20 nm) serial sections revealed that most of the tubulo-vesicular elements were separate structures not connected to the membrane of the vacuolar portion. Data here presented indicate that our ricin conjugate, like many "physiological' ligands and viruses, is internalized by receptor-mediated endocytosis via the coated pit-endosomal pathway.

摘要

我们制备了有毒植物蛋白蓖麻毒素与胶体金(粒径5纳米)的偶联物(Ri-Au),并将其用于Vero细胞单层培养的内化研究。Ri-Au偶联物非常稳定,在4.5 - 8.0的pH范围内,只有少量蓖麻毒素([125I]Ri)从金颗粒上释放出来。在37℃下2小时内,蓖麻毒素制剂([125I]Ri-Au)的细胞内降解非常少。细胞从培养基中结合天然蓖麻毒素([125I]Ri)和Ri-Au的比例相同,并且[125I]Ri和[125I]Ri-Au的毒性动力学([3H]亮氨酸细胞掺入量的减少)也具有可比性。在4℃时,电子显微镜显示Ri-Au在细胞表面的结合是连续且明显的。这种结合是特异性的,因为在0.1 M乳糖或1 mg/ml天然(未标记)蓖麻毒素存在下,4℃时几乎没有Ri-Au在细胞表面的结合。在将预先标记的细胞升温至37℃的最初30分钟内,表面相关的Ri-Au量显著减少(在40纳米切片中,每微米细胞表面从150个金颗粒减少到60个)。有被小窝和小泡参与了Ri-Au的内化,在37℃下5 - 30分钟内,Ri-Au被递送至内体系统的液泡和管状小泡部分,随后也被递送至溶酶体。对非常薄(约20纳米)的连续切片的分析表明,大多数管状小泡元件是独立的结构,未与液泡部分的膜相连。此处呈现的数据表明,我们的蓖麻毒素偶联物与许多“生理性”配体和病毒一样,通过有被小窝 - 内体途径经受体介导的内吞作用实现内化。

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